grant

The role of macrophage subpopulations in the rejuvenation of fracture repair

Organization DUKE UNIVERSITYLocation DURHAM, UNITED STATESPosted 1 Apr 2021Deadline 31 Dec 2026
NIHUS FederalResearch GrantFY2025AddressAgeAgingAllelesAllelomorphsApo E ReceptorApoE ReceptorApolipoprotein E ReceptorAutomobile DrivingBeta Cadherin-Associated ProteinBeta-1 CateninBone Marrow Blood-Deriving CellBone Marrow Blood-Forming CellBone Marrow CellsBone Marrow GraftingBone Marrow TransplantBone Marrow TransplantationCAP-18CAP18CAP18 lipopolysaccharide-binding proteinCRAMP proteinCUL-2Cell BodyCell DeathCell DifferentiationCell Differentiation processCell Growth in NumberCell MultiplicationCell ProliferationCell secretionCellsCellular ProliferationCellular SecretionCharacteristicsCirculationClinicalCnlpCyclic AMP ReceptorsDataDevelopmentDifferentiation in cell cultureErythroExposure toFIZZ3Found in Inflammatory Zone 3Fracture HealingGene ModifiedGenesIn VitroIn vitro cell differentiationKnowledgeLDL-Receptor Related Protein 1LL37LabelLineage TracingLow Density Lipoprotein Receptor-Related ProteinLow-Density-Lipoprotein Receptor-Related Protein-1MacrophageMarrow TransplantationMediatingMesenchymalMesenchymal DifferentiationMiceMice MammalsMorbidityMorbidity - disease rateMurineMusMyeloid ProgenitorMyeloid Progenitor CellsMyeloid Stem CellsOlder PopulationOperative ProceduresOperative Surgical ProceduresOsteoblastsPRO2286ParabiosisPhenotypePopulationProtein SecretionProteinsRETNRecombinantsRejuvenationRoleSourceSpleenSpleen Reticuloendothelial SystemSplenectomySurgicalSurgical InterventionsSurgical ProcedureTestingUndifferentiatedVascular blood supplyWorkYolk Sacadult animalagedaged animalaged animalsaged miceaged mouseagesalpha-2-Macroglobulin Receptoralpha2-Macroglobulin Signaling Receptoranimal old agebeta catbeta cateninblood supplybonebone fracture healingbone fracture repairbone healingbone repairbone wound healingcAMP Receptorscathelicidin antimicrobial peptidecathelin-like proteincathelin-related antimicrobial peptidecell lineage analysiscell lineage mappingcell lineage tracingcell lineage trackingcellular differentiationcellular lineage mappingcellular lineage trackingdefined contributiondevelopmentaldifferentiation in culturedifferentiation in vitrodrivingelderly animalelderly miceelderly patientexperimentexperimental researchexperimental studyexperimentsfetalfracture repairgene functiongene modificationgenetically modifiedhealingimprovedin vitro cellular differentiationin vivojuvenile animalmature animalmechanical propertiesmortalitymyeloid precursormyeloid stem and progenitor cellnecrocytosisnew drug treatmentsnew drugsnew pharmacological therapeuticnew therapeutic approachnew therapeutic interventionnew therapeutic strategiesnew therapeuticsnew therapynew therapy approachesnew treatment approachnew treatment strategynext generation therapeuticsnovel drug treatmentsnovel drugsnovel pharmaco-therapeuticnovel pharmacological therapeuticnovel therapeutic approachnovel therapeutic interventionnovel therapeutic strategiesnovel therapeuticsnovel therapynovel therapy approachold animalsold miceolder adultolder adulthoodolder groupsolder individualsolder patientolder personosseous wound healingosteoblast cell differentiationosteoblast differentiationosteoblastic differentiationprogenitorrecruitrepairrepairedresistinresponsescRNA sequencingscRNA-seqsingle cell RNA-seqsingle cell RNAseqsingle cell expression profilingsingle cell transcriptomic profilingsingle-cell RNA sequencingsocial rolesurgeryvascular supplyvitelline sacyoung animalβ-catenin
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Full Description

The pace of bone repair slows with aging, increasing the chance of developing a delayed union or non-union.
These complications are treated with surgical procedures causing significant morbidity and even mortality,
especially in older adults. Here we will build on our previous work using heterochronic parabiosis (in which two
mice of a different age share a blood supply) showing that exposure to a young circulation and young
macrophage cells rejuvenates fracture repair in older mice. In our preliminary data we used cell lineage tracing
analysis and parabiosis experiments to determine the developmental source of macrophage in fracture repair,
and found these derived from a subpopulation of cells of yolk sac origin. Interestingly these cells reside in the
spleen and are recruited through the circulation during bone repair. As mice age, this subpopulation of cells
becomes depleted. In this proposal we study the role of this cell population and the factors they produce in the
rejuvenation of fracture repair by undertaking the following aims:
1) Identify the role of macrophages derived from yolk sac progenitors in the rejuvenation of
fracture repair. Heterochronic parabiosis in which these cells can be labeled or depleted will be investigated
to define the contribution of young cells from this population of macrophage cells that can improve the quality
of fracture repair in older animals.
2) Determine the function of genes expressed in unique macrophage subpopulations present in
young mice in bone repair: We used single cell RNA sequencing and found a unique subpopulation of
macrophages cells present in bone repair in only young animals. Mice lacking genes which encode for
secreted proteins in various macrophage populations will be used in heterochronic parabiosis to determine
their contribution to the rejuvenation of fracture repair.
3) Define how specific macrophage populations and the proteins they secrete alter
mesenchymal differentiation in fracture repair. Our prior work showed an important role for beta-catenin in
mesenchymal cell differentiation and in fracture repair rejuvenation. Here we will use in-vitro approaches to
determine how specific subpopulations of macrophage cells and the proteins they secrete alter mesenchymal
cell differentiation in cells from young and old animals. There will be an initial focus on beta-catenin, but an
unbiased approach will be used as well.
This proposed work builds on our prior studies of rejuvenation by heterochronic parabiosis in fracture
repair. It will address critical gaps in our knowledge about the mechanism responsible for the rejuvenation
phenotype driven by heterochronic parabiosis. Our work will also identify a novel therapeutic approach to
address a critical clinical problem in older patients, delayed fracture healing.

Grant Number: 5R01AG072058-05
NIH Institute/Center: NIH
Principal Investigator: Benjamin Alman

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